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Revision as of 21:35, 1 July 2010 (view source) AndreasConstantinou (Talk | contribs) (New page: {{Stockholm/Top2}} = Andreas = == Preparation of competent BL21(DE3) cells == Competent cells were prepared as Team:Stockholm/1_July_2010) ← Older edit		Revision as of 22:14, 1 July 2010 (view source) AndreasConstantinou (Talk | contribs) Newer edit →
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	== Preparation of competent BL21(DE3) cells ==		== Preparation of competent BL21(DE3) cells ==
-	Competent cells were prepared as [[Team:Stockholm/1_July_2010]]	+	Competent cells were prepared as [https://2010.igem.org/Team:Stockholm/22_June_2010 previously described].
		+	;Modifications
		+	:*''Growth temperature was changed to 37°C''
		+	:*''Final OD(600) was 0.57''
		+
		+	== Preparation of LB agar plates with antibiotics ==
		+	* 50 ug/ml Km (20 plates)
		+	* 50 ug/ml Amp & 25 ug/ml Cm (10 plates)
		+	* 50 ug/ml Amp & 25 ug/ml Km (10 plates)
		+	''Plates were tested by plating with competent, non-transformed Top10 cells''
		+
		+	== Transformations ==
		+	Several different transformations were performed. Top10 cells were transformed with pSB1x3 BioBrick vectors. BL21(DE3) cells were transformed with SOD- and yCCS-carrying pEX vectors as well as with the pMA vector to test competence:
		+	==== Top10 ====
		+	*pSB1A3.BBa_J04450
		+	*pSB1C3.BBa_J04450
		+	*pSB1K3.BBa_J04450
		+	*pSB1AC3.BBa_J04450
		+	*pSB1AK3.BBa_J04450
		+	==== BL21(DE3) ====
		+	*pEX.SOD
		+	*pEX.yCCS
		+	*pMA.BBa_K157011
		+
		+	== Isolation of requested parts ==
		+	Our three requested parts BBa_J18930 (mCerulean; CFP), BBa_J18931 (mCitrine; YFP) and BBa_J18932 (mCherry; RFP) arrived as agar stabs. These were plated onto Amp plates according to [http://partsregistry.org/Help:Requesting_Parts_2009#Using_agar_stabs Registry instructions].

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Revision as of 22:14, 1 July 2010

Contents 1 Andreas 1.1 Preparation of competent BL21(DE3) cells 1.2 Preparation of LB agar plates with antibiotics 1.3 Transformations 1.3.1 Top10 1.3.2 BL21(DE3) 1.4 Isolation of requested parts

Andreas

Preparation of competent BL21(DE3) cells

Competent cells were prepared as previously described.

Modifications

• Growth temperature was changed to 37°C
• Final OD(600) was 0.57

Preparation of LB agar plates with antibiotics

• 50 ug/ml Km (20 plates)
• 50 ug/ml Amp & 25 ug/ml Cm (10 plates)
• 50 ug/ml Amp & 25 ug/ml Km (10 plates)

Plates were tested by plating with competent, non-transformed Top10 cells

Transformations

Several different transformations were performed. Top10 cells were transformed with pSB1x3 BioBrick vectors. BL21(DE3) cells were transformed with SOD- and yCCS-carrying pEX vectors as well as with the pMA vector to test competence:

Top10

• pSB1A3.BBa_J04450
• pSB1C3.BBa_J04450
• pSB1K3.BBa_J04450
• pSB1AC3.BBa_J04450
• pSB1AK3.BBa_J04450

BL21(DE3)

• pEX.SOD
• pEX.yCCS
• pMA.BBa_K157011

Isolation of requested parts

Our three requested parts BBa_J18930 (mCerulean; CFP), BBa_J18931 (mCitrine; YFP) and BBa_J18932 (mCherry; RFP) arrived as agar stabs. These were plated onto Amp plates according to Registry instructions.